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Shift Reagents for Multidimensional Ion Mobility Spectrometry-Mass Spectrometry Analysis of Complex Peptide Mixtures: Evaluation of 18-Crown-6 Ether Complexes

机译:用于复杂肽混合物的多维离子迁移谱-质谱分析的移位试剂:18-冠-6醚复合物的评估

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摘要

18-Crown-6 ether (18C6) is evaluated as a shift reagent for multidimensional ion mobility spectrometry-mass spectrometry (IMS-IMS-MS) analyses of tryptic protein digests. In this approach, 18C6 is spiked into the solution-phase mixture and noncovalent peptide-crown ion complexes are formed by electrospraying the mixture into the gas phase. After an initial mobility separation in the first IMS drift region, complexes of similar mobility are selected and dissociated via collisional activation prior to entering the second drift region. These dissociation products (including smaller complexes, naked peptide ions, charge transfer products, and fragment ions) differ in mobility from their precursor ion complexes and (in favorable cases) from one another, allowing the mixture to resolve further in the second IMS region. We estimate an IMS-IMS peak capacity of approx2400 when shift reagents are employed. The approach is illustrated by examining a tryptic digest of cytochrome c and by identifying a peptide out of a complex mixture obtained by digestion of human plasma proteins. Disadvantages arising from increased complexity of data sets as well as other advantages of this approach are considered.
机译:18-Crown-6醚(18C6)被评估为用于胰蛋白酶消化的多维离子迁移谱-质谱(IMS-IMS-MS)分析的转移试剂。在这种方法中,将18C6掺入溶液相混合物中,并通过将混合物电喷雾到气相中形成非共价肽-冠状离子络合物。在第一IMS漂移区中进行初始迁移率分离之后,在进入第二漂移区之前,通过碰撞激活选择并迁移具有类似迁移率的复合物。这些解离产物(包括较小的络合物,裸露的肽离子,电荷转移产物和碎片离子)在迁移率上不同于其前体离子络合物,并且(在有利的情况下)彼此之间也具有差异,从而使混合物在第二个IMS区域进一步分离。当使用移位试剂时,我们估计IMS-IMS峰容量约为2400。通过检查细胞色素c的胰蛋白酶消化物,并通过消化人类血浆蛋白而获得的复杂混合物中的肽来说明该方法。考虑了由于数据集复杂性增加而产生的缺点以及此方法的其他优点。

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